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Solid–solid phase transitions (SSPTs) are widespread naturally occurring phenomena. Understanding the molecular mechanisms and kinetics of SSPTs in various crystalline materials, however, has been challenging due to technical limitations. In particular, SSPTs in biomacromolecular crystals, which may involve large-scale changes and particularly complex sets of interactions, are largely unexplored, yet may have important implications for time-resolved crystallography and for developing synthetic biomaterials. The adenine riboswitch (riboA) is an RNA control element that uses ligand-induced conformational changes to regulate gene expression. Crystals of riboA, upon the addition of a ligand, undergo an SSPT from monoclinic to triclinic to orthorhombic. Here, solution atomic force microscopy (AFM) and polarized video microscopy (PVM) are used to characterize the multiple transition states throughout the SSPT in both the forward and the reverse directions. This contribution describes detailed protocols for growing crystals directly on mica or glass surfaces for AFM and PVM characterization, respectively, as well as methods for image processing and phase-transition kinetics analysis.

Supporting information

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AVI file https://doi.org/10.1107/S1600576721003137/te5074sup1.avi
Movie 1: Video of SSPT in a single riboA crystal in the presence of 10 mM ligand. The crystal was grown on a poly D-lysine-coated glass-bottom dish. Prior to recording, the dish was filled with 1.5 ml of stabilization buffer. After centring and focusing the crystal, the SSPT was initiated by adding 1.5 ml of 20 mM adenine-containing stabilization buffer. The video was recorded at 2456 x 1842 pixels and a rate of 0.27 seconds per frame. The total duration of the video is 45.9 seconds.

avi

AVI file https://doi.org/10.1107/S1600576721003137/te5074sup2.avi
Movie 2: 60 x 60 pixels ROI cropped from Movie S1 used for processing with OMAL PVM Analyzer


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